Fecal Carmine Red Protocol
Ian N Krout, Tim Sampson, Adam Hamilton
Abstract
This assay is used to determine whole gut transit time. Mice are given an oral gavage containing a known volume of bright red carmine dye. Mice are placed into empty cages and are then observed in 15-minute intervals until they produce a bright red fecal pellet. The time between gavage and pellet expulsion is the time the dye takes to travel down the length of the GI tract, which is influenced by gastric emptying, and small and large intestinal transit.
Steps
Pre-protocol
Prepare Carmine Red Soln. (see materials)
Autoclave Carmine Red Soln. if sterility is required. (i.e. microbiome analysis)
Shake well or stir on low heat to homogenize
Once resuspended, immediately aliquot into 1.5mL tubes and store in fridge to prevent spoilage.
Allow aliquots to come to room temperature prior to gavage.
Shake/vortex each right before gavage.
Day of Set-up
1.5mL Bring mice to the testing room for at least 1h 0m 0s prior to oral gavage to acclimate.
Day of Assay
Orally gavage mice with 100µL carmine red solution. Generally, soft-tipped, disposable (Instec FTP-20-30, or similar) feeding needles, attached to a 1mL slip-tip syringe.
Equipment
| Value | Label |
|---|---|
| Polypropylene Feeding Tubes for Rodents | NAME |
| Gavage Needle | TYPE |
| Instech Labs | BRAND |
| FTP-20-30 | SKU |
Record time of gavage for each mouse.
Following gavage, place animals back into home cage with cage mates, food, and water.
Allow animals to rest with food, water, in home cage for 1h 0m 0s (wildtype SPF mice will start
producing red pellets2h 0m 0s after gavage, while germ-free mice often take
longer tha4h 0m 0s ).
·Split individual mice into single-housed, clean (or sterile, if needed) cages, with no bedding , which will interfere with the observation of a red fecal pellet. Cover with cage top.
Assay can be set up with or without food as long as all comparable runs are done the same way. If
adding food, place 1-2 food pellets into a portion cup with water to create moistened chow (sterile if needed). Moistened chow reduces the risk of mice spilling water in the cage. Glass dishes can be used as cups to prevent flipping of the cups.
Optional: record number of pellets produced, cumulatively in 5-minute bins, for the first 30
minutes of separation (this can be informative of fecal output).
Every 0h 15m 0s, check cages for a bright red pellet. Can observe through sides (with pen light if needed) or by opening cage top. Placing the cages on a white sheet of paper, rather than a
black benchtop, will also make visualization easier. If food was provided, check in the portion cups for red pellets as well. Ensure that whichever method of observation is used, all animals are disrupted similarly (ie. all animals have their cages opened).
Pellets can be collected at each cage check, for water content or molecular assays, as long as
all cages are similarly disrupted during collection. Removing fecal pellets will also aid in determination of the first red fecal pellet produced.
Record time at which the first red pellet is observed for each mouse. For a normal, healthy adult mouse, this will be ~3-4hrs following gavage, but can range from 2-8+ hrs.
Once a red pellet is observed, return that mouse to its home cage.
To prevent stress associated with single-housing of mice, limit the single-housed portion of the assay to 6-8hrs, putting the maximum recordable transit time at 8-10hrs post-gavage.
If the maximum allotted time is reached without production of a red pellet, return the mouse to their
home cage, and record their transit time as the maximum.
Analysis
Compare the "time to red pellet" for each genotype or treatment group. This can be done pre- and post- exposures for toxicity assessments.
